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人甲状旁腺激素相关肽基因富含GC的启动子的鉴定与表征

Identification and characterization of a GC-rich promoter of the human parathyroid hormone-related peptide gene.

作者信息

Vasavada R C, Wysolmerski J J, Broadus A E, Philbrick W M

机构信息

Department of Internal Medicine, Yale University, New Haven, Connecticut 06510.

出版信息

Mol Endocrinol. 1993 Feb;7(2):273-82. doi: 10.1210/mend.7.2.8469240.

DOI:10.1210/mend.7.2.8469240
PMID:8469240
Abstract

The human PTH-related peptide (PTHrP) gene comprises eight exons spanning more than 15 kilobases of genomic DNA. The gene has a highly complex controlling region, which contains four alternatively spliced, noncoding exons and at least two putative promoters, one 5' of exon 1A (up-stream TATA element) and the other 5' of exon 2 (down-stream TATA element). To define important cis regulatory sequences of this gene, a functional dissection of PTHrP 5'-flanking DNA was initiated, using chimeric PTHrP-chloramphenicol acetyltransferase (CAT) constructs. This analysis was carried out in PTHrP-negative human renal carcinoma cells, so that RNA derived from transfected DNA could be studied without interference from endogenous PTHrP sequences. Of the initial series of constructs prepared, the most active was a 1.1-kilobase BamHI-HindIII PTHrP-CAT plasmid containing 350 basepairs of DNA 5' of exon 1C and extending into exon 3. Analysis of transfection products by RNase protection and primer extension revealed that this region contains a previously unrecognized promoter of the gene. This element is located immediately 5' of exon 1C, is active in transfected cells when cloned in isolation up-stream of the CAT gene, and appears to be functional in a number of cell lines and tissues on the basis of primer extension analysis. Unlike the other two PTHrP gene promoters, this element is GC rich and does not possess canonical TATA or CAAT sequences. The human PTHrP gene is one of a handful of genes that appear to use both TATA and GC-rich promoter elements.

摘要

人甲状旁腺激素相关肽(PTHrP)基因由八个外显子组成,跨越超过15千碱基的基因组DNA。该基因有一个高度复杂的调控区域,其中包含四个可变剪接的非编码外显子和至少两个推定的启动子,一个在1A外显子的5'端(上游TATA元件),另一个在2外显子的5'端(下游TATA元件)。为了确定该基因重要的顺式调控序列,利用嵌合的PTHrP-氯霉素乙酰转移酶(CAT)构建体对PTHrP 5'侧翼DNA进行了功能剖析。该分析在PTHrP阴性的人肾癌细胞中进行,这样转染DNA产生的RNA就可以在不受内源性PTHrP序列干扰的情况下进行研究。在最初制备的一系列构建体中,活性最高的是一个1.1千碱基的BamHI-HindIII PTHrP-CAT质粒,它包含1C外显子5'端350个碱基对的DNA,并延伸到3外显子。通过核糖核酸酶保护和引物延伸分析转染产物发现,该区域包含该基因一个以前未被识别的启动子。这个元件位于1C外显子的紧邻5'端,当单独克隆到CAT基因上游时在转染细胞中具有活性,并且根据引物延伸分析在许多细胞系和组织中似乎都有功能。与其他两个PTHrP基因启动子不同,这个元件富含GC,不具有典型的TATA或CAAT序列。人PTHrP基因是少数似乎同时使用TATA和富含GC的启动子元件的基因之一。

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